Host cells comprising Streptomyces clavuligerus chromosomal DNA fragments encoding enzymes for β-lactam antibiotic biosynthesis

ABSTRACT

DNA sequences obtained from  S. clavuligerus  ATCC 27064, recombinant vectors incorporating such sequences and hosts transformed with such vectors are disclosed. 
     The DNA comprises one or more genes coding for one or more enzymes involved in the biosynthesis of penicillin and cephalosporin β-lactams and such enzymes are expressed by hosts into which the recombinant vectors are transformed. 
     The DNA and the enzymes encoded thereby have utility in the preparation of penicillins and cephalosporins, both known and novel, possessing pharmacological, especially antimicrobial, activity.

This is a divisional of application Ser. No. 09/480,376, filed on Jan. 10, 2000 (now issued U.S. Pat. No. 6,709,859) which is a divisional of application Ser. No. 08/477,858, filed Jun. 7, 1995 (now issued patent U.S. Pat. No. 6,066,468), which is a continuation of application Ser. No. 08/292,060 filed Aug. 17, 1994 now abandoned; which is a continuation of application Ser. No. 08/147,041 filed Nov. 3, 1993 now abandoned; which is a continuation of application Ser. No. 08/004,785 filed Jan. 14, 1993 now abandoned; which is a continuation application of Ser. No. 07/632,630 filed Dec. 26, 1990 abandoned; which is a continuation of application Ser. No. 07/008,637 filed Jan. 29, 1987 abandoned, which claims benefit of foreign application Nos. GB 8602441 filed Jan. 31, 1986; GB 8604439 filed Feb. 22, 1986; and GB 8612057 filed May 17, 1986.

The present invention relates to recombinant DNA molecules, and in particular to recombinant vectors for use in the transformation of a microbial host which contain inserted DNA fragments carrying one or more genes coding for one or more enzymes involved in the biosynthesis of β-lactam antibiotics, especially penicillins and cephalosporins.

Progress in understanding the biosynthesis of β-lactam antibiotics produced by micro-organisms such as Streptomyces clavuligerus has been slow. Nevertheless it has been established that the biosynthetic pathways of certain penicillins and cephalosporins (including cephamycins) are closely related.

Isopenicillin N is an intermediate in the biosynthesis of both groups of compounds and is formed by the action of a ‘cyclase’ enzyme on the tripeptide δ(L-α-aminoadipyl)-L-cysteinyl-D-valine (sometimes referred to as LLD-ACV or, more simply, ACV as used hereinbelow). The intermediate isopenicillin N may be converted either into penicillin G or, by the action of an ‘epimerase’ enzyme, into penicillin N and it is from the latter that various cephalosporins and cephamycins may be derived by a multi-step pathway following an initial ring-expansion with an ‘expandase’ enzyme. A recent summary of the state of the art is given by J. F. Martin and P. Liras in Trends in Biotechnology, 1985, 3, 39-44. Thus, in the biosynthesis of Cephamycin C, penicillin N is converted into deacetoxycephalosporin C which is then converted by a dioxygenase enzyme into desacetylcephalosporin C.

The latter is O-caroamoylated to give O-carbamoyldesacetylcephalosporin C, which is then converted into Cephamycin C. It is probable, in the light of work by J. D. Hood et al. (J. Chem. Soc., Chem. Commun, 1983, pages 1187-1188 and references therein) that the 7α-methoxy group in Cephamycin C is introduced in two steps, i.e. via the action of a 7-hydroxylase enzyme on O-carbamoyldesacetylcephalosporin C to give the 7α-hydroxy derivative, followed by subsequent methylation.

As is now well known, by means of recombinant DNA techniques, it is possible to insert into a host cell DNA carried on a vector with the result that the transformed host may become endowed with the capacity to synthesise whatever protein(s) or enzyme(s) the gene(s) carried on the insert DNA may encode. (For a full discussion of recombinant DNA methodology, and a glossary of the terms used therein, see ‘Principles of Gene Manipulation’ by R. W. Old and S. B. Primrose, 3rd Edition, Blackwell Scientific Publications, 1985).

The isolation and expression in E. coli of the isopenicillin N synthetase (cyclase) gene from C. acremonium has recently been reported by S. M. Samson et al (Nature, 1985, 318, 191-194).

In order to clearly define the invention reference is made to the accompanying drawings in which:

FIG. 1(a) is an endonuclease restriction map of S. clavuligerus ATCC 27064 chromosomal DNA (I) coding for genes involved in penicillin and cephalosporin biosynthesis;

FIG. 1(b) is an endonuclease restriction map of the portion of the DNA (I) contained in a plasmid designated pBROC 138;

FIG. 1(c) is an endonuclease restriction map of the portion of the DNA (I) contained in a plasmid designated pBROC 137;

FIG. 1(d) is an endonuclease restriction map of a portion of the DNA (I) contained in a plasmid designated pBROC 303;

FIG. 2 is an endonuclease restriction map of plasmids pBROC 137 and pBROC 138; and

FIG. 3 is an endonuclease restriction map of plasmid pBROC 303.

Accordingly, the present invention provides DNA (I) or a restriction fragment derived therefrom containing one or more genes coding for one or more enzymes involved in the biosynthesis of penicillin and cephalosporin β-lactams, the said DNA having the configuration of restriction sites hereinunder shown in FIG. 1(a).

The present invention further provides a recombinant vector capable of transforming a host cell, which vector contains insert DNA or a restriction fragment derived therefrom containing one or more genes coding for one or more enzymes involved in the biosynthesis of penicillin and cephalosporin β-lactams, the said DNA having the configuration of restriction sites hereinunder shown in FIG. 1(a).

Accordingly, in another aspect of the invention there is provided a host cell transformed with the recombinant vector or the invention. Suitably such host cells are micro-organisms, preferably E. coli or Streptomycetes, for example S. lividans 66 (DSM 1567).

As will be readily appreciated by those skilled in the art, it may not be convenient, or desired, to utilize the whole DNA segment (I) shown in FIG. 1(a) in the recombinant vector of the invention. Accordingly, suitable restriction fragments derived from the full length DNA (I) shown in FIG. 1(a) may be used as the insert DNA provided said suitable fragments contain one or more intact genes involved in the biosynthesis of penicillins and cephalosporins.

The restriction fragments according to the invention may be derived from the DNA segment (I) by cleavage with appropriate restriction enzymes by known methods.

Particularly preferred DNA fragments include those having the configuration of restriction sites shown in FIG. 1(b), FIG. 1(c) or FIG. 1(d) hereinbelow.

In FIGS. 1 to 3 the abbreviations ClaI, BclI etc. are conventional abbreviations for restriction endonucleases (see Old and Primrose, loc.cit.), and the approximate length in kilobases (Kb) of the DNA, as determined by sizing experiments carried out by agarose gel electrophoresis, is indicated. It should be understood that FIGS. 1 to 3 indicate the approximate positions of the restriction enzyme cleavage sites, as determined by such sizing experiments, and are not necessarily intended to show all the possible restriction sites present on the DNA illustrated.

The DNA characterized in FIG. 1(a), or a suitable restriction fragment derived therefrom such as the fragments illustrated in FIGS. 1(b), 1(c) and 1(d) may be ligated to any vector capable of transforming any host cell in which the gene(s) coating for enzyme(s) involved in the biosynthesis of penicillins or cephalosporins may be expressed.

It will be understood that for the DNA or the invention to be expressed in such a host cell, the said DNA may either carry its own native promoter sequence which is recognised by an RNA polymerase of the host cell, or may be ligated to another suitable promoter sequence in a suitable fashion, or may be cloned at an appropriate restriction site, and in the correct translational reading frame, into a vector incorporating a suitable promoter sequence.

Suitable host cells in which the DNA of the invention may be expressed include E. coli, Penicillium species, Cephalosporium species, or Streptomyces species such as S. clavuligerus and S. lividans.

Normally the vector into which the DNA of the invention may be cloned is a plasmid, for example a plasmid derived from a Streptomycete, or is a temperate or virulent phage.

An example of a suitable vector is pIJ 702 (molecular weight 8.9 megadaltons), a high copy number plasmid described by Katz, E. et al in J. Gen. Microbiol., 1983, 129, 2703-2714, and available from the John Innes Institute, Norwich, England.

An example of a suitable temperate phage is that known as ØC31, described by Lomovskaya, N. O., Chater, K. F., Mkrtumian, N. M., in Bacterial. Rev., 1980, 44, 206-229.

The recombinant vectors of the invention may be prepared by ligating the insert DNA characterized in FIG. 1(a), or a restriction fragment derived therefrom, to the chosen (linearized) vector by any convenient method, for example by direct combination of cohesive ends, homopolymer tailing, or by means of a linker or adapter molecule.

It will be appreciated that recombinant vectors prepared according to the above methods may contain the insert DNA in one of two possible orientations. Recombinant vectors containing both orientations are included within the scope of the invention.

Suitable recombinant vectors are plasmids containing the DNA fragments characterized by the configuration of restriction sites shown in FIGS. 1(b), 1(c) and 1(d) hereinbelow. Preferred recombinant vectors are those in which:

-   i) the DNA fragment shown in FIG. 1(b) is inserted into the BglII     site of pIJ 702 (the construct is referred to hereinbelow as pBROC     138); or -   ii) the DNA fragment shown in FIG. 1(c) is inserted into the BglII     site of pIJ 702 (the construct is referred to hereinbelow as pBROC     137); or -   iii) the DNA fragment shown in FIG. 1(d) is inserted into the BglII     site of pIJ 702 (the construct is referred to hereinbelow as pBROC     303).

To prepare the DNA of the invention, a random array of DNA fragments may be generated by partial digestion of S.clavuligerus ATCC: 27064 total cellular DNA by any convenient restriction enzyme. The endonuclease Sau 3AI (abbreviated hereinbelow to Sau 3A) and its isoschizomers are particularly suitable for this purpose.

The DNA fragments may then be size-fractionated on a sucrose gradient and fragments of length >3 Kb, preferably <15 Kb, may be isolated. Preferred fragments are of 4-14 Kb in size. The DNA fragments may then be ligated by conventional ‘shot-gun’ methods to a suitably cleaved vector, for example pIJ 702, and after recircularisation the recombinant vector may be transformed into a strain of S. clavuligerus which lacks the capability to produce Cephamycin C.

A suitable strain of S. clavuligerus for this purpose is S. clavuligerus NCP-5 which was deposited in the Beecham Culture Collection under the accession number BCC1 on 29th Jan. 1986 and later transferred to the National Collection of Industrial and Marine Bacteria, Aberdeen, Scotland, the deposit (NCIB 12208; filing date 19th Feb. 1986) being made under the terms of the Budapest Treaty on the International Recognition of the Deposit of Micro-organisms for the Purposes of Patent Procedure.

Accordingly, S. clavuligerus NCIB 12208 forms another aspect of the present invention.

The derivation and characteristics of S. clavuligerus NCP-5 (S. clavuligerus NCIB 12208) are as follows.

Derivation of S. clavuligerus NCP-5

Breaking out a sample of S. clavuligerus ATCC 27064 showed a variety of morphologies. Fourteen different types were recognised. One of these was isolated as S. clavuligerus SC-2. When cultured, S. clavuligerus SC-2 itself shows a variety of morphologies. From an example of the ‘small’ variety a ‘large’ colony variant was spontaneously derived, and designated S. clavuligerus NCP-5.

Taxonomy of S. clavuligerus, NCP-5

The taxonomical and morphological properties of S. clavuligerus NCP-5 were round to be essentially similar to those of S. clavuligerus ATCC 27064, a description of which may be found in U.S. Pat. No. 3,862,008 and also in Higgens, C. E. and Kastner, R. E., Int. J. Systematic Bacteriol., 1971, 21, 326-331. The method of culturing S. clavuligerus NCP-5 is similar to that described for S. clavuligerus ATCC 27064 in British Patent Specification No. 1 508 977.

The transformants obtained by the ‘shot gun’ methods hereinbefore described may be screened for their ability to produce Cephamycin C by bringing them into contact with a micro-organism sensitive to that compound and examining the growth characteristics of the said micro-organism. A suitable micro-organism for this purpose is A. faecalis (deposited in the National Collection of Industrial and Marine Bacteria under the Accession Number NCIB 8156 and also available to the public from the Beecham Culture Collection (accession number BCC2) at any time on request). For the purposes of the screening procedure the A. faecalis may be conveniently grown on agar plates, and a complementation assay may be carried out by inserting plugs of the transformants into the plates by conventional methods known in the art.

Transformants identified as ‘positive’ by their ability to produce zones or growth inhibition on media freshly seeded with a Cephamycin-sensitive micro-organism such as A. faecalis may be isolated and the recombinant vectors contained therein may be isolated from each ‘positive’ colony by conventional methods. On digestion of the recombinant vectors with suitable restriction enzymes, the S. clavuligerus DNA inserted into each vector may be identified, sized, and ‘mapped’ by cleavage with a variety of restriction enzymes in the conventional manner in order to check that it contains the DNA of the invention.

Two or more ‘overlapping’ inserts so isolated (i.e. inserts having common DNA) which are wholly or partly embraced within the DNA of the invention but are too small to contain intact genes involved in the biosynthesis of penicillins and cephalosporins may often be fused together by cleavage at a common restriction site followed by ligation (e.g. with DNA ligase) in the conventional manner to give, for example, the insert DNA of pBROC 137 and pBROC 138 or a suitable restriction fragment derived therefrom as hereinbefore defined.

The DNA (I) illustrated in FIG. 1(a) may be isolated by using the S. clavuligerus DNA of pBROC 137 or pBROC 138 to identify, by colony hybridization, E. coli cells carrying cosmids made from S. clavuligerus ATCC 27064 total cellular DNA and pHC79 (Hohn, B and Collins, J. (1980), Gene, 11, 291). The plasmid pBROC 303 may then be constructed from pIJ 702 and the DNA fragment illustrated in FIG. 1(d) [obtained from DNA (I)] by a simple subcloning procedure.

The production of enzymes involved in the biosynthesis of penicillins and cephalosporins may be achieved by re-inserting the DNA of the invention into a suitable vector, for example pIJ 702, and transforming a suitable host micro-organism, for example S. lividans 66 (DSM 1567), with the thus formed recombinant vector.

Particularly valuable enzymes so produced include those known in the art (J. F. Martin and P. Liras, loc.cit.) as ‘cyclase’ or isopenicillin N synthetase (capable of converting ACV into isopenicillin N), ‘expandase’ or deacetoxycephalosporin C synthetase (capable of converting penicillin N into deacetoxycephalosporin C), ‘epimerase’ or penicillin N synthetase (capable of converting isopenicillin N into penicillin N), and O-carbamoyldesacetylcephalosporin C-7-hydroxylase (capable of converting both O-carbamoyldesacetylcephalosporin C and cephalosporin C into their respective 7-hydroxy derivatives). Such enzymes of S. clavuligerus ATCC 27064, or any other proteins with the capability to bring about the synthesis of penicillins and cephalosporins, form another aspect of the present invention when produced by the transformed hosts of the invention. Preferably the proteins or enzymes are obtained in highly purified form.

Such proteins or enzymes may be isolated and purified by conventional methods.

The DNA of the invention and vectors containing same may find use in many areas of industrial activity. That also applies to host micro-organisms transformed with said vectors and the enzymes they express. For example the DNA may be utilised as a hybridization probe to identify and isolate related or overlapping genes present on the total cellular DNA of S. clavuligerus ATCC 27064 and of other micro-organisms which produce enzymes of similar structure and specificity.

Accordingly, the invention also provides the use of DNA (I) or any fragment thereof capable of hybridising to the DNA of a β-lactam antibiotic producing micro-organism for the purpose of isolating genes involved in β-lactam antibiotic biosynthesis in that organism.

Recombinant vectors containing the DNA of the invention may be of value, when transformed into suitable hosts, in the production of genetically modified micro-organisms which synthesize increased amounts of valuable antibiotics such as Cephamycin C, or in the generation of novel or hybrid antibiotics via the process of gene transfer (see for example D. A. Hopwood et al., Nature, 1985, 314, 642-644). Enzymes encoded by the DNA of the invention may be used, for example, in cell-free systems especially when immobilised on suitable solid supports to prepare known β-lactam antibiotics from their natural precursors or novel β-lactams from ‘unnatural’ precursors obtained, for example, by chemical synthesis.

The DNA of the invention or a fragment thereof (not necessarily carrying an intact gene) may be combined, either by recombinant DNA techniques or by natural recombination processes, with a fragment of a gene involved in β-lactam biosynthesis to produce a hybrid gene capable of directing the synthesis of a hybrid enzyme. Such enzymes may be used in the production of novel antibiotics by processes analogous to those hereinbefore described.

The DNA of the invention may also be modified by the known techniques or site-directed mutagenesis (in a manner analogous to that described, for example, by G. Winter et al., Nature, 1982, 299, 756-758; or by Zoller and Smith, Nucleic Acids Research, 1982, 10, 6487-6500) to give DNA in which specific mutations and/or deletions have been effected. The mutated DNA may be used to obtain an increased yield (or titre) of known β-lactam antibiotics from a suitable host micro-organism that already produces such compounds. The mutated DNA may also be used to obtain novel or hybrid antibiotics by gene transfer, or used in the production of mutant enzymes (muteins) which may be used in the production of novel antibiotics by analogous processes to those hereinabove described.

It will be understood that such mutated DNA is contemplated within the scope of the present invention.

The invention will now be illustrated by the following Examples.

EXPERIMENTAL

Preparation 1. Isolation of 4-15 kb Size Pieces of Sau 3A Digested S.clavuligerus 27064 DNA

-   (a) Total cellular DNA was prepared from S.clavuligerus 27064 in the     following manner: -   i) Spores of S.clavuligerus 27064 were inoculated into 2 shake     flasks of tryptone Soya Broth Maltose growth medium (30 ml/250 ml     spring shake flask—Trytone Soya Broth 30 g/l., Maltose 10 g/l) and     incubated for 48 hours at 26° C. (240 rpm). -   ii) The mycelium was harvested by centrifugation at 10,000 G. -   iii) The supernatant fraction was poured off and the pellets     resuspended in 10 ml of lysing solution (50 mM Tris pH 8.5, 50 mM     Na₂ EDTA, 15% sucrose, lysozyme 3 mg/ml) and incubated for 1 hour at     37° C. -   iv) 0.5 ml Sodium Lauryl Sulphate (10% solution) containing 2 mg     Proteinase K (ex SIGMA chemicals) was added and incubation continued     for 15 minutes whereupon more SLS/Prot K solution was added and     incubation was continued for a further 15 minutes. -   v) The DNA was spooled out on a glass rod after the addition of Na     Acetate (to 0.3 M) and ice cold Ethanol (2 vols). This was repeated     several times to give a translucent viscous preparation of DNA. -   (b) Partial Sau 3A digestion of chromosomal DNA from S.clavuligerus     27064.     -   180 μg of total cellular DNA was incubated with 12 units of Sau         3 A restriction enzyme (NEW ENGLAND BIOLABS SUPPLIED) in the         recommended buffer for 30 minutes at 37° C. The reaction was         stopped by denaturing the enzyme at 70° C. When the extent of         DNA digestion was examined by agarose gel electrophoresis it was         found that the fragments ranged in size from 15 kb to 0.16 kb. -   (c) Fractionation of Sau 3A partially digested DNA on a sucrose     gradient 40% to 10% w/v.     -   A sucrose gradient (40-10%) was prepared in a 13 ml centrifuge         tube as described in ‘Genetic Manipulation of Streptomyces—A         Laboratory Manual—authors; D. A. Hopwood et. al., published by         the John Innes Foundation 1985’.     -   The Sau 3A partial digest of S.clavuligerus 27064 DNA (100 μg in         0.5 ml) was carefully layered on top of the sucrose gradient and         the system centrifuged for 30,000 rpm (10⁵ gav) for 21 hours.     -   The tube was removed from the centrifuge and fractions (400 μl)         were collected from a pierced hole in the bottom of the tube. 5         μl samples of these fractions were examined by gel         electrophoresis and those fractions shown to contain DNA of 4-14         kb in size were collected together. In this way 12 μg of Sau 3A         digested DNA of 4-14 kb in size was obtained.         Preparation 2. Preparation of pIJ 702 Vector DNA Suitable for         Cloning Sau 3A Fragments of S.clavuligerus 27064 DNA -   (a) Isolation of plasmid DNA.     -   Spores of S.clavuligerus 27064: pIJ 702 were inoculated into         TSB/Maltose medium in shake flasks (see Preparation 1(a) for         make up of medium). Thiostrepton was added to 2.5 μg/ml to         maintain plasmid stability. The micro-organism was grown for 48         hours at 26° C. pIJ 702 (Ref: Katz, E., et. al. J. Gen.         Microbiol. (1983) 129 2703-2714) plasmid was isolated from the         mycelium by use of the Neutral Lysis Procedure (see Hopwood et.         al. 1985 loc.cit.). In this way 50 μg of pIJ 702 DNA was         isolated. -   (b) BglII Digestion of pIJ 702 DNA from S.clavuligerus 27064.     -   30 μg of pIJ 702 DNA was digested with BglII restriction enzyme         (100 units as supplied by Amersham International) in a total         volume of 400 μl of recommended restriction buffer for 30         minutes at 37° C.     -   The reaction was stopped by incubation at 70° C. for 30 minutes.     -   Examination of a sample of the reaction mix on agarose gel         electrophoresis (0.7% gel) showed that all of the closed         covalent circular (CCC) plasmid initially present had been         converted to linear form. -   (c) Calt intestinal alkaline phosphatase (CIAP) treatment of BglII     digested pIJ 702 DNA.     -   This was carried out as described in ‘Molecular Cloning—A         Laboratory Manual, Maniatis, T. et. al. publisher by Cold Spring         Harbour Laboratory (1982)’     -   Examination of the CIAP treated DNA in the presence of T4 DNA         ligase showed that it would no longer self-ligate after the         enzymatic dephosphorylation had been carried out.         Preparation 3. Ligation of Sau 3A Digested Total Cellular DNA of         S.clavuligerus 27064 with BglII Digested, CIAP Treated pIJ 702         DNA.

To each of 12 containers containing 1 μg of Sau 3A digested S.clavuligerus 27064 chromosomal DNA (4-14 kb) in 50 μl of water was added 100 μl of BglII digested, CIAP treated pIJ 702 (0.5 μg/pot) in buffer to give final concentrations of 1.5 μg DNA/150 μl, Tris. HCl pH 7.5 (66 mM), MgCl₂ (6.6 mM), Dithiothreitol (10 mM) and Adenosine Triphosphate (0.4 mM). T4 DNA LIGASE (0.1 unit—as supplied by Amersham International) was added to each pot and the systems incubated at 15° C. for 72 hours before transformation into the required recipients.

Preparation 4. Formation of a Library of S.clavuligerus NCP-5. pIJ 702/27064 Clones

-   (a) Testing the ligated DNA in S.lividans 66 for frequency of     inserted DNA into pIJ 702 and size of DNA inserts.     -   1.5 μg of ligated DNA (4-14 KD Sau 3A generated fragments of         S.clavuligerus 27064 ligated with BglII digested, CIAP treated         pIJ 702 prepared from S.clavuligerus 27064) was dissolved in 10         μl TE buffer (1 mM Na₂ EDTA, 10 mM Tris. HCl pH 8.2) and used as         2×5 μl aliquots in the transformation of 2×100 μl volumes of         S.lividans 66 (DSM 1567) protoplasts (10¹⁰         protoplasts/ml—prepared as described in ‘Genetic Manipulation of         Streptomyces—A Laboratory Manual’—in the presence of 25%         polyethylene glycol (average molecular weight 1000).     -   After transformation the protoplasts were plated out at         dilutions of up to 10⁻⁴ on R2YE agar (see Hopwood et. al., loc         cit).     -   After incubation at 32° C. for 24 hours the plates were         overpoured with soft nutrient broth (SNBA) agar (8 g Difco         Nutrient Broth/l, 3 g agar/l containing Thiostrepton antibiotic         (500 μg/ml) to select for plasmid bearing colonies and also         containing L-Tyrosine (1 g/l) to detect those colonies bearing         plasmids with inserts in the mel gene of pIJ 702.     -   After several days of growth the frequency of black colonies         (less than 2%) and the transformation efficiency of the ligated         DNA (9.3×10³ transformants/μg DNA) could be ascertained by         counting.

Plasmids were prepared from 10 of the white S.lividans 66 colonies in the manner previously described (Preparation 2a). These plasmid preparations were digested with BclI restriction enzyme with subsequent agarose gel electrophoresis in order to determine the size of DNA inserts.

-   -   It was determined in this fashion that the average size of DNA         cloned was 5 kb.

-   (b) Transformation of a Ligated DNA Sample into S.clavuligerus NCP-5     (S. clavuligerus NCIB 12208)     -   1.5 μg of ligated DNA was transformed in 2×5 μl of T.E. buffer         into 2×100 μl of S.clavuligerus NCP-5 protoplasts (10¹⁰         protoplasts/ml, prepared as in Hopwood et. al., (1985) loc. cit.         The transformed protoplasts were regenerated at 26° C. on R5         agar (100 g sucrose/l, 10 g dextrin/l, 5.1 g MgCl₂.6H₂O/l, 1 g         Casamino acids/l, 0.05 g MgSO₄.7H₂O/l, 2.5 g L-Arginine HCl/l, 1         ml trace elements/l, 20 g Oxoid Technical Agar no. 3/l, 0.05 g         KH₂PO₄/l, 3.7 g CaCl₂.2H₂O/l, 5.7 g TES buffer pH 7.2 g/l. Trace         elements solution consisted of FeSO₄.7H₂O 1 g/l, MnCl₂.4H₂O 1         g/l, ZnSO₄.7H₂O 1 g/l). Thiostrepton resistant colonies were         selected by overlaying with SNBA (as described in Preparation         4a) containing Thiostrepton (50 μg/ml) after 48 hours of         regeneration. After a further 72 hours the transformed colonies         were individually scraped, in arrays onto a nutrient agar         suitable for antibiotic production (M5D⁺ agar containing Dextrin         10 g/l, K₂HPO₄ 1 g/l, MgSO₄.7H₂O 1 g/l, (NH₄)₂SO₄ 1 g/l,         Industrial Chalk 4 g/l, Trace Element solution 1 ml/l, Agar 20         g/l, yeast extract 2 g/l and Bacteriological peptone 2.5 g/l.         The trace element solution consists of FeSO₄.7H₂O 0.1%,         MnCl₂.4H₂O 0.1% and ZnSO₄.7H₂O 0.1%) and containing Thiostrepton         (2.5 μg/ml).     -   4500 NCP-5 colonies which displayed Thiostrepton resistance         conferred by pIJ 702: S.clavuligerus 27064 DNA plasmids were         obtained in this manner.         Preparation 5. Screening the NCP-5: pIJ 702/S.clavuligerus 27064         Library for Production of Cephamycin C.

After 10 days of growth on M5D⁺ agar at 26° C., 8 mm diameter agar plugs were cut from each of the mycelial patches and placed upon DST agar (40 g Oxoid DST agar/l water) which had been freshly seeded with Alcaligenes faecalis ATCC 8750/NCIB 8156. (See Claridge, C. A. and Johnson, D. L. (1962) Antimicrob. Ag. Chemother. 682-686)). This organism is sensitive to certain cephalosporins such as cephalosporin C and cephamycin C but not penicillin N even in the presence of the low levels of clavulanic acid produced by NCP-5 under the growth conditions used, consequently NCP-5 which produced penicillin N and clavulanic acid only normally gives no zone of inhibition of growth on A.faecalis NCIB 8156 whereas its parent S.clavuligerus strain does (as it produces penicillin N, clavulanic acid and Cephamycin C). The antibiotic from the plugs was allowed to diffuse into the DST/A.faecalis agar and after overnight incubation at 37° C. the A.faecalis growth examined for zones of antibiosis.

In this way, possible production of Cephalosporin antibiotics by any of the members of the library of clones was searched for. Two of the clones labelled NCP-5/36/5 and NCP-5/10/7 were found to give zones of antibiosis against A.faecalis.

Preparation 6. Examination of the Plasmid Content of NCP-5/36/5 and NCP-5/10/7.

-   (a) Physical Examination of the Plasmids     -   Plasmid preparations were made from NCP-5/36/5 and NCP-5/10/7 as         described in Preparation 2a. It was possible to isolate several         micrograms of plasmid material from 30 ml cultures of each of         the two positives. Restriction enzyme site mapping showed         clearly that only a single species of plasmid was present in         NCP-5/36/5 and also only a different single species in         NCP-5/10/7. Restriction Mapping (see FIG. 1) suggested that the         plasmids pBROC 137 and pBROC 138 isolated from NCP-5/36/5 and         NCP-5/10-/7 respectively contained approximately 5.7 kb and         approximately 5.8 kb DNA inserts in pIJ 702. The two DNA inserts         appeared to contain a common fragment of approximately 2.7 kb as         suggested by mapped restriction enzyme sites and this was         subsequently proved by showing extensive hybridization of the         respective ³²P labelled fragment of pBROC 138 to the predicted         portion of pBROC 137 DNA using Southern analysis. -   (b) Reintroduction of the plasmids pBROC 137 and pBROC 138 into     NCP-5.     -   100 nanogram amounts of pBROC 137 and pBROC 138 DNA were used to         retransform S.clavuligerus NCP-5. The transformed colonies were         isolated and subsequently tested upon A.faecalis bioassay plates         as described in Preparation 5.     -   It was apparent that at least 90% of all of the NCP-5 colonies         retransformed with pBROC 137 or pBROC 138 were now able to give         zones of antibiosis on A.faecalis. This confirmed that the DNA         present in pBROC 137 and pBROC 138 contained genetic information         able to repair the mutation incurred with NCP-5.         Preparation 7. The Assay of Novel Enzymatic Activities Conferred         upon Streptomyces Lividans 66 by pBROC 137, pBROC 138, and pBROC         303

100 nanogram quantities of pBROC 137 DNA, pBROC 138 DNA and pBROC 303 DNA transformed into S.lividans 66 (as in Preparation 4a).

Cultures of S.lividans 66: pBROC 137, S.lividans 66 pBROC 138, and S.lividans 66: pBROC 303 were grown in shake flasks of YEME (30 ml glucose 10 g/l, Sucrose 340 g/l, malt extract 3 g/l, Bacteriological Peptone 5 g/l, yeast extract (Oxoid) 3 g/l, containing Thiostrepton antibiotic at 50 μg/ml. The cultures were grown for 48 hours at 32° C. at 240 rpm. Mycelium was harvested by centrifugation at 10,000 g and washed with Tris. HCl buffer pH 7.0 (0.05 M). The mycelium was recentrifuged and the pellet resuspended in 2.5 ml Tris. buffer. Cell disruption was carried out by use of a French Pressure Cell at 1000 psi and the broken cell preparations centrifuged at 10⁵ g for 60 minutes to furnish a cell free, particulate free soluble enzyme preparation.

-   (a) Demonstration of Expandase Enzymic Activity

Enzyme preparations from S.lividans 66: pIJ 702, S.lividans 66: pBROC 137 and S.lividans 66: pBROC 138 were used in ring expansion assay systems (as described in Jensen, S. E., Westlake, D. W. S. and Wolfe, S., (1983) Antimicrob. Ag. Chemother. 24(3) 307-312) to determine the presence of deacetoxycephalosporin C synthetase.

Utilizing the E.coli ESS/Penicillinase (DIFCO Penicillinase Concentrate 10⁴ u/ml) bioassay system described by these authors it could be shown that the S.lividans 66: pIJ 702 extracts were unable to transform Penicillin N to penicillinase resistant antibiotics whereas the extracts from S.lividans 66 pBROC 137 and S.lividans 66: pBROC 138 were able to carry out that transformation. S.lividans 66: pBROC 137 enzyme extracts were able to carry out a substantial transformation of the penicillin N in the assay system to penicillinase resistant antibiotic whereas the enzyme extract from S.lividans 66: pBROC 138 exhibited much lower activity in this respect. Subsequently the ring expansion assays were chromatographed on cellulose t.l.c. plates (Butanol/Acetic Acid/Water, 3/1/1) together with authentic samples of penicillin N, deacetoxy cephalosporin C and deacetyl cephalopsorin C. Bioassay of the chromatograms on E.coli ESS/Difco Penicillinase containing agar showed, after overnight incubation at 37° C., that S.lividans 66: pBROC 137 enzyme extracts had transformed penicillin N into deacetoxy Cephalosporin C whereas extracts of enzyme from S.lividans 66: pIJ 702 did not. No deacetyl cephalosporin C was identified as being synthesized from penicillin N by any of the cell extracts. (Rf of deacetoxy cephalosporin C=0.55; Rf of deacetyl Cephalosporin C=0.39.). (Penicillin N is not detected due to presence of penicillinase).

-   (b) The Conversion of iso-Penicillin N to a chemical form more     active against E.coli ESS.

Using the iso-Penicillin N epimerase assay developed by Jensen, S. E. et. al. (Can. J. Microbiol. (1983) 29(11) 1526-1531) it was possible to demonstrate that a cell free, particulate free enzyme extract (as in Preparation 7a) from S.lividans 66: pBROC 137 was able to convert iso-Penicillin N to a chemical form at least ten times more active against E.coli ESS than iso-Penicillin N itself. A similar extract from S.lividans 66: pIJ 702 was unable to do this.

-   (c) The Conversion of O-Carbamoyl Desacetyl Cephalosporin C and     Cephalosporin C to their 7-Hydroxy derivatives by cell free     preparations of S.lividans 66: pBROC 303.

Cell free preparations of S.lividans 66: pBROC 303 (0.9 ml) were incubated at 22° C. with Sodium Ascorbate (2.8 mM), Ferrous Sulphate (0.045 mM), α-ketoglutarate (1 mM), Potassium Chloride (7.5 mM), Magnesium Sulphate (7.5 mM), Tris-hydrochloride pH 7.0 (0.05 M), and either O-Carbamoyl Desacetyl Cephalosporin C (0.5 mM) or Cephalosporin C (0.5 mM) in a final volume of 1.2 ml.

After 2 hours of incubation, 25 μl of Glacial Acetic Acid was added with shaking and a de-proteinated supernatant was obtained by centrifugation (10,000 G for 5 minutes). This liquid was absorbed onto a QAE-Sephadex column (1 ml volume). The resin was washed with 250 μl of water and 200 μl of 0.2M NaCl.

The cephalosporins were eluted from the resin with a further 250 μl of 0.2 M NaCl.

20 μl samples of these concentrated reaction products were analysed by High Performance Liquid Chromatography using C₁₈ reverse-phase Microbondapak columns. The mobile phase for the separation of O-Carbamoyl Desacetyl Cephalosporin C from 7-Hydroxy O-Carbamoyl Desacetyl Cephalosporin C was 0.1 M NaH₂PO₄, pH 3.2. To separate Cephalosporin C from 7-Hydroxy Cephalosporin C the pH of the mobile phase was increased to 4.2 Elution was carried out at 2 ml/minute with U.V. detection at 260 n.m.

In this manner it was possible to demonstrate approximately 50% conversion of O-Carbamoyl Desacetyl Cephalosporin C (retention time 5.7 minutes) to its 7-Hydroxy derivative (retention time 3.0 minutes) and approximately 35% conversion of Cephalosporin C (retention time 18.2 mins) to 7-Hydroxy Cephalosporin C (retention time 6.6 minutes). Extracts of S.lividans 66: pIJ 702 were unable to carry out these transformations.

Preparation 8. Sodium Lauryl Sulphate/Polyacrylamide Gel Electrophoresis of Proteins Produced by S.lividans 66: pBROC 137 and S.lividans 66 pBROC 138.

Volumes (5 μl, 10 μl) of cell free, particulate free extracts of S.lividans 66: pBROC 137, S.lividans 66 pBROC 138 and S.lividans 66: pIJ 702 (as in Preparation 7a) were treated with sodium lauryl sulphate (SLS) to denature the proteins in solution and chromatographed by SLS/12% Polyacrylamide Gel Electrophoresis using the method of Laemmli, U. K. (Nature (1970) 227 392). Staining with Coomassie Brillant Blue revealed that as could be judged from proteins of known molecular weight co-chromatographed, the extracts from S.lividans 66: pBROC 137 and S. lividans 66: pBROC 138 displayed a protein of approximately 29,500 Daltons which was either not present or very much fainter in the extract from S. lividans 66: pIJ 702. The extract from S.lividans 66: pBROC 137 also displayed a prominently staining protein band at approximately 60,000 Daltons in size.

Preparation 9. The Isolation, Characterization and Subcloning of DNA from the S.clavuligerus Chromosome Contiguous with that DNA Contained in pBROC 137 and pBROC 138

a) Construction of a library of S.clavuligerus ATCC 27064 DNA in pHC 79.

10 μg of pHC 79 DNA (Holm, B. and Collins, J (1980) Gene 11, 291-298) was digested to completion with restriction enzymes SalI and BamHI. A further 10 μg or pHC 79 DNA was digested to completion with Eco RI and BamHI. To isolate the required ‘cosmid arms’ both digests were fractionated on a sucrose gradient (10-40%). The yield of each cosmid arm was >5 μg.

100 μg of S.clavuligerus ATCC 27064 chromosomal DNA was partially digested with Sau 3AI and fractionated on a sucrose gradient (10-40%). Fractions containing restriction fragments >30 Kb and <50 Kb were pooled thus providing approximately 10 μg of Sau 3AI fragments in this size range. These fragments were ligated to the cosmid arms at a molar ratio of 1:1:1 (DNA concentration 200 μg ml⁻¹). After 24 hours the ligation mix was packaged in vitro into lambda phage. (Phage lambda packaging extracts and protocol supplied by Amersham International PLC). Transfection of E.coli DHI (Low, B. (1968) PNAS 60, 161-167) yielded 5×10⁷ transfectants/μg packaged DNA.

-   b) Isolation of DNA segment (I) from the S.clavuligerus ATCC 27064     DNA library and subcloning this DNA into pIJ 702.

5000 E.coli DHI colonies containing pHC 79 with S.clavuligerus ATCC 27064 DNA inserts were immobilized and lysed on nitrocellulose filters. The 1.2 Kb BclI—KpnI ended fragment from pBROC 137 was isolated and nick translated. This fragment was used to probe the filters by standard colony hybridization techniques. Seven hybridizing colonies were obtained, one of which contained DNA segment (I) illustrated in FIG. 1(a).

Subcloning fragments of DNA segment (I) was effected by first digesting 10 μg of this cloned DNA with BamHI. 5 μg of the vector, pIJ 702, was digested with BglII and treated with CIAP to prevent recircularization The BamHI generated fragments were ligated to the BglII digested, CIAP treated pIJ 702 at a molar ratio of 2:1 respectively and a DNA concentration of 50 μg ml⁻¹. After incubation at 15° C. for 24 hours 0.5 μg of ligation mix was transformed into S.lividans 66 and 2×10⁵ transformants/μg obtained. Screening the transformants permitted the isolation of pBROC 303 together with the other BamHI fragment clones. 

1. A host cell comprising a recombinant vector comprising a DNA segment having a nucleotide sequence endogenous to Streptomyces clavuligerus ATCC 27064 and the configuration of restriction endonuclease sites shown in FIG. 1(a), or a restriction fragment derived therefrom, said segment or fragment comprising genes encoding one or more enzymes selected from the group consisting of penicillin N synthetase, deacetoxycepahalosporin C synthetase, and O-carbamoyldesacetylcepahalosporin-C-7-hydoxylase, and wherein the host cell is selected from the group consisting of E. coli, Penicillium, Cephalosporium, and Streptomyces.
 2. A host cell according to claim 1 in which the DNA segment or fragment has the configuration of restriction endonuclease sites shown in FIG. 1(b), FIG. 1(c), or FIG. 1(d).
 3. A host cell according to claim 1 in which the vector comprises the plasmid pIJ
 702. 4. A host cell according to claim 1, in which the recombinant vector or vectors is selected from the group consisting of pBROC 137, pBROC 138 and pBROC
 303. 5. A host cell comprising at least one recombinant vector comprising a DNA segment having a nucleotide sequence endogenous to Streptomyces clavuligerus ATCC 27064 and having the configuration of restriction endonuclease sites shown in FIG. 1(a), or a or a restriction fragment derived therefrom, said segment or fragment comprising genes encoding one or more enzymes selected from the group consisting of penicillin N synthetase, deacetoxycephalosporin C synthetase, and O-carbamoyldesacetylcephalosporin C-7-hydroxylase, wherein the host cell is E. coli, Penicillium and Cephalosporium.
 6. A host cell according to claim 5 in which the DNA segment or fragment has the configuration of restriction endonuclease sites shown in FIG. 1(b), FIG. 1(c), or FIG. 1(d).
 7. A host cell according to claim 5 in which the vector comprises the plasmid pIJ
 702. 8. A host cell according to claim 5, in which the recombinant vector or vectors is selected from the group consisting of pBROC 137, pBROC 138 and pBROC
 303. 9. A method for expressing an enzyme selected from the group consisting of penicillin N synthetase, deacetoxycepahalosporin C synthetase, and O-carbamoyldesacetylcepahalosporin-C-7-hydoxylase in a recombinant host cell, said method comprising culturing a transformed host cell of claim 4 or claim 5 under conditions suitable for expression of said enzyme. 